Mineral Analysis, In Vitro Evaluation of Alpha-Amylase, Alpha-Glucosidase, and Beta-Galactosidase Inhibition, and Antibacterial Activities of Juglans regia L. Bark Extracts

In traditional medicine, various parts of the plant Juglans regia L. are used to treat several pathological conditions including diabetes and infectious and periodontal diseases. This includes the bark of Juglans regia. The present study is aimed at evaluating for the first time the mineral composition, investigating the antidiabetic and antibacterial properties of Moroccan J. regia bark, and finally determining the correlations between the chemical composition of the tested extracts and their biological activities. The mineral composition was determined using inductively coupled plasma atomic emission spectroscopy. Then, nine extracts were prepared by different methods and modalities of extractions and investigated for their antidiabetic activities, via tests of inhibition of alpha-amylase, alpha-glucosidase, and beta-galactosidase enzymes, and for their antibacterial activities against six strains involved in infectious diseases and periodontology. Finally, the correlation between the chemical compositions of the different extracts prepared and their antidiabetic and antibacterial potencies was determined by Principal Component Analysis (PCA). J. regia is an important source of mineral elements, mainly Fe (19849.8), K (3487.8), Mg (2631.03), and P (691.02) mg/kg plant material. All the extracts of J. regia possess antidiabetic activity, and in particular, the macerated acetone extract gave the highest inhibitory activity against alpha-amylase (IC50 value of 5445.33 ± 82.58 μg/mL), alpha-glucosidase (IC50 value of 323.7 ± 1.71 μg/mL), and beta-galactosidase (IC50 value of 811.2 ± 8.32 μg/mL). For the results of antibacterial activity, the macerated acetone extract at the concentration of 80 mg/mL was found to be the most active by inducing inhibition diameters of 12, 17, 18, 11, 14.5, and 16 mm against Escherichia coli, Proteus mirabilis, Pseudomonas aeruginosa, Staphylococcus aureus, Bacillus subtilis, and Listeria innocua, respectively. PCA allowed us to deduce that the extracts richer in polyphenols, in particular, the two acetone and ethanol macerates, have a better antidiabetic activity against alpha-glucosidase as well as a better antibacterial activity. The results of the present study revealed that the aqueous and organic macerate extracts showed a better antidiabetic activity and justified the use of J. regia bark as an antibacterial and antiseptic agent in traditional Moroccan medicine in the treatment of dental affections.


Introduction
Diabetes mellitus is characterized by chronic hyperglycemia and disorders of carbohydrate, lipid, and protein metabolism associated with absolute or relative deficits in insulin action and/or secretion [1,2]. The World Health Organization (WHO) has predicted that between 2014 and 2045, the number of people with diabetes will increase from 422 million to approximately 629 million [3]. Diabetes (mainly type 2 dia-betes) is seeing its prevalence explode in developing countries. In Morocco, between 2011 and 2015, the number of diabetics increased from 1.5 million people to more than 2 million, an increase of 25% in 5 years. 80% of diabetes cases are type 2 and mainly are people over 40 years of age and obese [4]. However, recent studies have shown a significant increase in the number of children and adolescents with this disease, which may be associated with bad eating habits and a lack of physical activity. This leads to increasing rates of obesity, which is considered a risk condition for the development of type 2 diabetes [5].
Faced with this situation, the population has sought alternative and less expensive treatments for the diabetes disease, including the use of plants as a remedy for this disease, because the medicinal plant can have considerable hypoglycemic properties [5]. The literature analysis showed that several studies reported the benefits of different herbal treatments on several metabolic changes caused by type 2 diabetes. These studies also show the positive effects of plant extracts on normalizing body weight and decrease glucose levels, total cholesterol, and triglycerides [6][7][8].
In addition to diabetes, infectious diseases are a public health problem because of their frequency and severity. However, periodontal disease is defined as a bacterial infection that affects and destroys the supporting tissues of the teeth (gingiva, periodontal ligament, cementum, and alveolar bone) through an accumulation of bacterial biofilm on the surface of the teeth. This biofilm is defined as a complex microbial community of oral bacteria organized in supraand subgingival biofilm [9]. Therefore, treatment of this biofilm with antimicrobial agents may be beneficial and necessary. Antiseptic agents, such as chlorhexidine, cetylpirinidium chloride, and fluorides, in different formulations (mouthwashes, gels), are often and still used in periodontology to potentiate the eradication of periodontal pathogens [10,11]. However, the majority of these agents have limited subgingival efficacy, reaching only partially the subgingival biofilm and inaccessible inflamed tissue. Also, the appearance of adverse effects (dental staining, taste alteration, etc.) and bacterial resistance have often been described following prolonged use of these chemical agents [12]. Faced with these many obstacles in the use of available antibacterials, it is essential to search for new effective antibacterial substances with a broad spectrum of action. One of the strategies for this research is to explore plants used in traditional medicine.
Eastern Morocco, and more particularly the region of Taza, is characterized by a significant phytodiversity, of which several plants are used in both the treatment of diabetes and dental diseases. Among these plants, Juglans regia is one of the most commonly used in traditional medicine for the treatment of diabetes [13,14]. Previous studies in Iran have even reached the stage of clinical trials by formulating 100 mg capsules of Juglans regia leaf extract in the treatment of diabetic patients [15][16][17]. Other studies have shown that the leaves have antidiarrheal, anthelmintic, and antiseptic properties and are used in the treatment of skin inflammation, ulcers [18], and cancer [19][20][21]. Orhan et al. reported the neuroprotective effect of extracts prepared from the leaves and fruits of Juglans regia harvested in Turkey [22]. Boulfia et al. have reported the antioxidant activity of aqueous and organic Moroccan Juglans regia bark extracts [23]. In addition, the bark of Juglans regia is reputed to have antibacterial and antiseptic activities, acting against bad breath and bleeding gums according to an ethnopharmacological survey that we conducted in the region of Taza, Morocco [24]. Phytochemical analysis of Juglans regia has been the subject of different research studies. NirmlaDevi et al.
The present study represents the continuation of our experimental studies on the Moroccan Juglans regia L. bark, the first part of which was devoted to the study of the effects of the use of different extraction solvents with different polarities, aqueous and organic extraction methods, and hot and cold extraction modalities by maceration on the presence and content of secondary metabolites and the antioxidant activity [23].
In the present work, we were interested in determining for the first time the mineral composition of the Moroccan Juglans regia L. bark and in evaluating the antidiabetic activity via three tests of inhibition of the enzymes alpha-amylase, alpha-glucosidase, and beta-galactosidase of its aqueous and organic extracts (ethanolic, acetonic, and diethyl ether) prepared hot by Soxhlet extraction and cold by maceration. Subsequently, we were also interested in studying their antibacterial activity by the method of diffusion on disc and in determining the minimum inhibitory and bactericidal concentrations of the extracts which proved to be active. Finally, we used Principal Component Analysis (PCA) to reveal the correlations between the chemical composition of the tested extracts and the results of the study of its antidiabetic and antibacterial activities.

Mineral Content.
According to the method of Arora et al. [31], the mineral composition of Juglans regia bark was investigated. Mineral elements (potassium (K), calcium (Ca), magnesium (Mg), sodium (Na), phosphorus (P), copper (Cu), iron (Fe), selenium (Se), strontium (Sr), and zinc (Zn)) were determined using inductively coupled plasma atomic emission spectroscopy (ICP-AES) (HORIBA Jobin Yvon). Thus, 0.1 mg of J. regia bark was digested with nitric acid and perchloric acid (25% : 75%) solution, before being incinerated at 110°C, then brought back dry until the mineralization was discolored on a sand bath. The residue was dissolved in 10 mL HCL (5%), and the contents were filtered through 0.45 μm porosity filters until a clear solution was obtained. The sample solution was made up to a final volume of 25 mL with distilled water and analyzed by atomic absorption spectrophotometry (ICP-AES) (HORIBA Jobin Yvon).

Qualitative and Quantitative Phytochemical Analysis.
To determine the chemical composition of J. regia bark, two analyses have been conducted; the first one was aimed at investigating the presence or absence of the main secondary metabolites (alkaloids, tannins, saponins, anthraquinones, flavonoids, quinones, sterols, and anthracenosides) by staining and/or precipitation reactions, and the second one sought to quantify the content of polyphenols, flavonoids, and tannins present in aqueous and organic extracts of J. regia bark [23].
2.6. Evaluation of the Antidiabetic Effect 2.6.1. Alpha-Amylase Inhibitory Activity. The alpha-amylase inhibitory potentials were investigated by reacting different concentrations of the extracts with alpha-amylase enzyme and starch solution, according to the method of Wickramaratne et al. [32]. A mixture of 200 μL of samples and 200 μL of 0.02 M sodium phosphate buffer (pH = 6:9) containing the enzyme alpha-amylase (2 U/mL) was incubated at 30°C for 10 min. Then, 200 μL of 1% starch solution in 0.02 M sodium phosphate buffer (pH = 6:9) was added to the reacting mixture. Therefore, the reaction mixture was incubated at 30°C for 3 min. Thereafter, 200 μL of dinitrosalicylic acid (DNS) was added, and the reaction mixture was incubated in a boiling water bath at 85-90°C for 10 min. Then, the reaction mixture was diluted by adding 5 mL of distilled water, and absorbance was measured at 540 nm in the spectrophotometer (SPECUVIS2 UV/Vis, No: HF1309003). Acarbose was used as a positive control.
The alpha-amylase inhibitory activity was expressed as percent inhibition and was calculated as follows: where A1 refers to the absorbance of the control (enzyme +buffer), A2 refers to the absorbance of control blank (buffer without enzyme), A3 refers to the absorbance of the sample (enzyme + extract), and A4 is the absorbance of sample blank (extract without enzyme).
2.6.2. Alpha-Glucosidase Inhibitory Activity. The inhibitory potency of J. regia extracts against alpha-glucosidase was evaluated by measuring the formation of 4-nitrophenol by alpha-glucosidase after reaction with 4-p-nitrophenyl-α-Dglucopyranoside (pNPG) according to the method of Lordan et al. [33]. Thus, the reaction mixture containing 150 μL of extracts at various concentrations and 100 μL of alphaglucosidase solution (0.1 U/mL) was preincubated at 37°C for 10 min. Subsequently, 200 μL of 1 mM pNPG solution in sodium phosphate buffer (0.1 M/pH = 6:7) was added and incubated at 37°C for 30 min. The reaction was terminated by adding 1 mL of sodium carbonate solution (Na 2 CO 3 /0.1 M), and the absorbance was measured at 405 nm. Acarbose was included as a positive control. The percent inhibition of alpha-glucosidase was determined as described in the alpha-amylase assay, and the IC 50 values were determined.
2.6.3. Beta-Galactosidase Inhibitory Activity. The betagalactosidase inhibition activity was evaluated using the method of Maruhn in 1976 [34]. For the inhibition of the beta-galactosidase enzyme, a mixture of 150 μL of various extract concentrations and 100 μL of sodium phosphate buffer (0.1 M/pH = 7:6) containing the solution of enzyme beta-galactosidase (1 U/mL) was incubated at 37°C for 10 min. Then, we added 200 μL of 2-nitrophenyl β-D-galactopyranoside (1 mM) solubilized in sodium phosphate buffer (0.1 M/pH = 7:6). Reaction mixtures were incubated at 37°C for 30 min. After incubation, 1 mL of Na 2 CO 3 was added to stop the reaction, and absorbance was measured at 410 nm. Quercetin was used as a positive control. The percent inhibition of beta-galactosidase was determined as described in alpha-amylase and alpha-glucosidase assays. The concentration of the sample that inhibits the enzyme by 50% was evaluated.

Preparation of Bacterial Suspensions.
To prepare the bacterial suspensions, three to four well-isolated colonies 3 BioMed Research International were selected and emulsified in a tube containing sterile saline solution to have turbidity near that of McFarland 0.5 standards; the suspensions were then diluted in tubes containing sterile saline solution to have a final concentration of 10 8 CFU/mL. An inoculum of 100 μL of each bacterial suspension was plotted in petri dishes, each containing 20 mL of Müeller-Hinton's agar, and left hanging for 5 min before inserting the discs.

Disc Diffusion
Method. The experimental protocol consisted of depositing a sterile Whatman paper disc (6 mm in diameter) impregnated with different concentrations of the prepared extracts of J. regia bark (20, 40, and 80 mg/mL) dissolved in 10% of DMSO. The dishes were left for 15 min at room temperature and then incubated at 37°C for 20 h. After incubation, the antibacterial effect was evaluated by measuring the inhibition zones in millimeters against the tested bacterial strains [35]. The experiments were repeated three times. Negative controls were performed by DMSO at 10%, while tetracycline and amikacin were used as positive controls.

Determination of Minimum Inhibitory Concentration (MIC)
. This technique consists of making successive dilutions in a liquid culture medium (Müeller-Hinton) in microplates of 96 sterile wells, from a stock solution of the extracts to be tested and whose concentration is known (80 mg/mL). To these dilutions, a microorganism suspension (10 μL) with a concentration of 10 8 CFU/mL was added to each well. Afterward, the plates were incubated at 37°C for 24 hours. Then, 10 μL of MTT solution (3-(4,5-dimethyl-2-thiazolyl)-2,5-diphenyl-2H-tetrazolium bromide) was added to each well, and the plate was reincubated for 15 minutes at 37°C. The results were read visually, and the appearance of a purple stain shows bacterial growth. The lowest concentration which had no visible growth after 24 h incubation was considered as the MIC [36].

Determination of Minimum Bactericidal Concentration (MBC).
To determine the MBC values, well solutions with an extract concentration equal to or higher than the MIC values were used. 10 μL from each well was subcultured on nutrient agar (Müeller-Hinton's agar) in petri dishes. The bacterial cultures were incubated at 37°C for 24 h. The minimum concentration that had no visible growth on agar plates after 24 h incubation was considered as the MBC.

Statistical Analysis.
The results were expressed as the mean ± standard error. Nonlinear regression analysis was adopted to determine the IC 50 values of the three assays (alpha-amylase, alpha-glucosidase, and beta-galactosidase assays). The data were analyzed by one-way analysis of variance (one-way ANOVA), Turkey, and the procedure consisted of comparing all pairs of columns for the significance of difference. A difference in the mean values of p < 0:05 was considered to be statistically significant. Analysis was performed with GraphPad Prism® 5.0 software. Principal Component Analysis (PCA) was performed by the XLSTAT software.

Mineral
Composition of Juglans regia L. Bark. According to our bibliographic research, the present study represents the first international study dedicated to the evaluation of the mineral composition of J. regia bark. The results of this study are expressed in milligrams per kilogram of plant material (mg/kg) and are represented in Table 1. This shows that J. regia bark is an important source of mineral elements, with very high contents of Fe (19849. 3.2. Evaluation of the Antidiabetic Effect of Juglans regia L. Bark 3.2.1. Alpha-Amylase Inhibitory Activity. According to our bibliographic research, there are many studies of the antidiabetic activity of J. regia leaves, but few studies evaluated this activity on the bark of J. regia. The present study represents for the first time the results of alpha-amylase, alpha-glucosidase, and beta-galactosidase inhibition of aqueous and organic extracts of J. regia bark and are presented in Table 2. From this table, we noticed that for the alphaamylase inhibition assay, aqueous extracts are less active than organic extracts. For the aqueous extracts, the extract prepared by infusion was the most active with an IC 50 of about 8689:66 ± 318:23 μg/mL, twice as active as that prepared by decoction (IC 50 = 16161 ± 62:61 μg/mL). For the organic extracts, the macerated acetone showed the best alphaamylase inhibition activity with an IC 50 of about 5445:33 ± 82:58 μg/mL. Compared to the reference standard, acarbose exhibited an IC 50 in the range of 616:33 ± 6:58 μg/mL which remains significantly active than the aqueous and organic extracts of J. regia bark.
3.2.2. Alpha-Glucosidase Inhibitory Activity. The results obtained from the evaluation of the alpha-glucosidase inhibition activity of the aqueous and organic extracts of J. regia are listed in Table 2 and show that the two extracts prepared by Soxhlet extraction and by cold maceration by the acetone solvent proved to be the most active with a nonsignificant difference (acetone extract: IC 50 = 306:9 ± 1:88 μg/mL; macerated acetone: IC 50 = 323:7 ± 1:71 μg/mL). The aqueous extract prepared by cold maceration showed an interesting hypoglycemic effect with an IC 50 of about 414:46 ± 13:98 μg/mL. All tested extracts were found to be less active than the reference standard, acarbose, which showed an IC 50 value of 195 ± 5 μg/mL which is significantly different from the aqueous and organic extracts of J. regia (P < 0:05).

3.2.3.
Beta-Galactosidase Inhibitory Activity. The different extracts prepared from the J. regia bark were tested for their hypoglycemic activity by the beta-galactosidase inhibition assay, and the results obtained are represented in Table 2. These showed that all the extracts tested have a betagalactosidase inhibition capacity with a significant difference (P < 0:05) between aqueous and organic extracts and that the latter is more active than the aqueous extracts. The aqueous  Table 3; we can note that the organic extracts prepared from J. regia bark exhibit a wide spectrum of the zone of inhibition which varies depending on the strain tested, the extract tested, and the concentration used. For the disc diffusion method, an extract is considered active when it induces a zone of inhibition greater than or equal to 10 mm [37]. According to Table 3, all extracts were active against all tested strains. Thus, the macerated acetone extract at the concentration of 80 mg/mL was found to be the most active by inducing the inhibition diameters of 12, 17, 18, 11, 14.5, and 16 mm on Escherichia coli, Proteus mirabilis, Pseudomonas aeruginosa, Staphylococcus aureus, Bacillus subtilis, and Listeria innocua, respectively. Similarly, the macerated diethyl ether extract at the same concentration showed high antibacterial power with inhibition diameters of 14, 21.5, 10, 14.5, 20, and 11 mm on Escherichia coli, Proteus mirabilis, Pseudomonas aeruginosa, Staphylococcus aureus, Bacillus subtilis, and Listeria innocua, respectively. It should be noted that the inhibition diameters induced by all these extracts remain higher than those of the reference antibiotic, amikacin, which showed no zone of inhibition against Escherichia coli, Proteus mirabilis, and Staphylococcus aureus strains. Similarly, tetracycline was active only against Escherichia coli, Proteus mirabilis, and Staphylococcus aureus strains with inhibition diameters of 13, 23, and 13 mm, respectively.

Minimal Inhibitory Concentration (MIC) and Minimal
Bactericidal Concentration MBC). The purpose of the microdilution method is to evaluate minimum inhibitory concentrations and determine the lowest concentration of an antibacterial agent necessary to inhibit the growth of a microorganism.
The present study allowed us to determine the minimum inhibitory concentration of the different organic extracts of J. regia bark and then to determine the minimum bactericidal concentration of our extracts, which allowed us to quantify and compare these results with those of the disc diffusion method, but also to characterize the nature of the effect revealed by an extract on a given microorganism. Table 4 summarizes the results obtained from the minimum inhibitory and bactericidal concentrations of organic extracts of J. regia. According to this table, we notice that     The MBC/MIC ratio was also calculated to highlight the nature of the antibacterial effect of the extracts tested. When this ratio is lower than 4, the extract is considered a bactericidal extract, and when it is higher than 4, it is considered a bacteriostatic extract [38].

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According to Table 4, it appears that all the organic extracts tested do not have a bactericidal effect but rather a bacteriostatic power; it is the case of the macerated acetone which exerts a bacteriostatic effect against 4 strains, namely, Escherichia coli, Pseudomonas aeruginosa, Staphylococcus aureus, and Listeria innocua, followed by the ethanolic extract with a bacteriostatic effect against 3 strains, namely, Escherichia coli, Pseudomonas aeruginosa, and Listeria innocua. The other extracts have a bacteriostatic power on one or two strains (Table 4).

Principal Component Analysis (PCA).
To determine the correlations between the chemical composition [23] and the different pharmacological activities evaluated in this work, namely, antidiabetic and antibacterial, we calculated the correlation matrix based on the results of the determination of polyphenols, flavonoids, and tannins and the results of the antidiabetic and antibacterial activities represented as variables, and the individuals are the nine aqueous and organic extracts of J. regia bark (Table 5).
From Table 5, we noticed that the richer the extract is in polyphenols, the better the correlation with the alphaglucosidase inhibition test and the antibacterial activity represented by the Pseudomonas aeruginosa strain with a correlation coefficient of r = 0:7904 and 0.9595, respectively. The extracts that are rich in tannins (macerated diethyl ether and macerated acetone) show positive correlations with the strains of antibacterial activity of Escherichia coli, Staphylo-coccus aureus, and Bacillus subtilis with a correlation coefficient of r = 0:9511, r = 0:7969, and r = 0:8818, respectively. A weak correlation was obtained between alpha-amylase and alpha-glucosidase enzyme inhibition tests and flavonoid content with correlation coefficients of r = 0:3819 and r = 0:0787, respectively.
The distribution of the tests of antidiabetic and antibacterial activity with the organic extracts of J. regia bark on the first two axes F1 and F2 of the PCA are presented in Figure 1. According to the latter, we notice that the twoaxis F1 and F2 explain 74.29% of the retained information; the first component F1 explains 51.52% of the total information, and the second component F2 shows 22.78% of the total information.
The F1 axis is mainly constituted by the positive correlation between polyphenols, tannins, and bacterial strains Escherichia coli, Proteus mirabilis, Pseudomonas aeruginosa, Staphylococcus aureus, Bacillus subtilis, and Listeria innocua. The F2 axis is formed mainly by the alpha-glucosidase inhibition test (Figure 1).

Mineral Composition of Juglans regia L. Bark.
According to our literature search, there have been no previous studies that evaluated the mineral content of J. regia bark and our study is the first one that assayed the mineral elements present in this part of the plant.
The walnut (J. regia L.), which belongs to the Juglandaceae family, is one of the nuts commonly found in the Mediterranean diet. Recently, the walnut has been considered a natural functional food of great economic interest because of its nutritional and medicinal benefits. Moreover, the nut contains many beneficial compounds, such as polyunsaturated fatty acids and proteins. The beneficial effect of nut consumption against many diseases has been reported, including protection against diabetes [39]. In addition, the bark of J. regia is a part of the plant widely used by the population in traditional medicine, because of its anti-inflammatory, anticancer, depurative, diuretic, and laxative properties     [25]. The antioxidant properties of J. regia bark have been studied and reported in our previous work [23]. In addition, the mineral elements of a plant can influence its medicinal properties. Therefore, the present study is aimed at quantifying the content of mineral elements present in the bark of J. regia. From Table 1, we noticed that J. regia is an important source of both macroelements (calcium (Ca), potassium (K), magnesium (Mg), sodium (Na), and phosphorus (P)) and microelements (copper (Cu), iron (Fe), strontium (Sr)) which play an important role in human diet due to their antioxidant power. Indeed, calcium is the most abundant mineral in the body, with 1000 to 1500 g found in adults; it is involved in many reactions in our cells at the enzyme level. Phosphorus plays a role in the constitution of cells. Sodium is the predominant element in the blood and the extracellular fluids of the body; it determines the water balance of the organism and the hydration of the cells (with potassium) and plays a role in maintaining the acid-base balance. Magnesium has an important physiological role; it stimulates the formation of antibodies, necessary in many enzyme systems, especially those related to energy production [40]. Our results are in agreement with the results of the mineralogical analysis of the walnut conducted by Tapia  In comparison with another plant collected in the region of Taza, named Leopoldia comosa, the investigations of the mineral composition shows that the bulb of Leopoldia comosa has very high contents of Fe and K with values, respectively, of 33552 and 1843.14 mg/kg of plant matter, followed by P (756.36 mg/kg), Na (439.65 mg/kg), Cu (303.9 mg/kg), Mg (272.37 mg/kg), and Ca (20.55 mg/kg of plant matter) [42]. The richness of the bulb of Leopoldia comosa by mineral elements can explain their food use in the Mediterranean countries.

Antidiabetic
Activity of Juglans regia L. Bark. Due to the lack of studies evaluating the hypoglycemic properties of J. regia bark, the present study seeks to evaluate and document these properties and subsequently compare the activity of different parts of the same plant that would allow the use of the right part of the plant to have the best activity.
From our study, we noticed that all the extracts of J. regia bark showed inhibition activity of alpha-amylase, alpha-glucosidase, and beta-galactosidase enzymes and that this activity varies from aqueous to organic extracts and also from one enzyme to another, which can be explained by the use of different extraction modalities that we have adopted in our study and which consequently impacted the presence or absence of secondary metabolites with varying concentrations between aqueous and organic extracts and also between extracts prepared with Soxhlet extraction or cold by maceration. Similarly, the choice of using different tests to evaluate the antidiabetic activity influenced the results obtained by 9 BioMed Research International allowing to differentiate between the extracts tested according to their mechanisms of action.
For the alpha-amylase assay, the infused extract was the most active of the aqueous extracts with an IC 50 = 8689:66 ± 318:23 μg/mL, and for the organic extracts, the macerated acetone exhibited the greatest inhibitory power with an I C 50 = 5445:33 ± 82:58 μg/mL.
In comparison with a plant from the region of Taza studied in our laboratory under the same experimental conditions, Bouabid et al. reported that the two aqueous and methanolic macerate extracts prepared from the underground part of Atractylis gummifera L. (Asteraceae) were found to have an inhibitory effect of alpha-amylase enzyme with an IC 50 , respectively, in the order of 1000 ± 0:055 μg/ mL and 557 ± 0:013 μg/mL. Similarly, for the alphaglucosidase test, the aqueous and methanolic macerates presented IC 50 values of the order of 1461 ± 0:047 μg/mL and 743 ± 0:017 μg/mL. For the beta-galactosidase test, the aqueous macerate presented with an IC 50 of the order of 2230 ± 0:012 μg/mL, while on the other hand, the methanolic macerate presented with an IC 50 of the order of 2443 ± 0:071 [43]. These results are better than those obtained for extracts prepared from Juglans regia bark (Juglandaceae), which can be explained by the difference of the botanical family and therefore the presence of other chemical families. The results of the hypoglycemic power of Atractylis gummifera extracts justify their traditional uses by the population in the treatment of diabetes [13]. Several previous works have demonstrated that phenolic compounds can influence carbohydrate metabolism at different levels, improving postprandial glycemic levels, fasting blood glucose, insulin secretion, and insulin sensitivity, being that a strategy for the prevention of type 2 diabetes is aimed at limiting the rate of blood glucose uptake through the intestines [44,45]. In comparison with other studies performed on J. regia, Rahimzadeh et al. [46] reported that the aqueous macerated extract prepared from the leaves of this plant harvested in Iran has a very high alpha-amylase inhibitory power with an IC 50 value of 320 ± 0:07 μg/mL, which is still more than 40 times more active than the one we found for the aqueous macerate in our study with an IC 50 = 13424:33 ± 284:55 μg/mL. The result can be explained by the geographical variation of the harvest of the plant, the methods, and modalities of extractions used, and also the part of the plant that can influence the medicinal properties of a plant. Another study performed on the leaves of J. regia reported that the hydroalcoholic extract of this plant harvested in Iran at the concentration of 200 mg/kg of rat weight resulted in a significant decrease in blood glucose, glycosylated hemoglobin, LDL, triglycerides, and total cholesterol and a significant increase in insulin and HDL levels [17]. Similarly, the study by Javidanpour et al. reported that the methanolic extract of J. regia leaves harvested in Iran significantly decreased the level of glucose (p < 0:05) and glycosylated hemoglobin (p = 0:001) in streptozotocin-induced diabetic rats [47].  8, 8.75, and 0 mm on the strains previously described [48]. Another study carried out in Iran by Bakhtiari and Khalafi [49] on the hydroalcoholic macerated extract of J. regia bark showed a zone of inhibition of 16.2, 14, 14.2, and 13.3 mm, respectively, on Staphylococcus aureus, Pasteurella multocida, Mannheimia haemolytica, and Streptococcus spp. at the concentration of 250 mg/mL. These results are still higher than those of the study that was conducted by Zakavi et al. [48]. This can be explained by the difference in the extraction modality and the choice of solvent used for extraction. In comparison with our study, our results are superior to those obtained by Zakavi et al. [48]; we found a 10 mm zone of inhibition on Staphylococcus aureus and only at the concentration of 80 mg/mL of the ethanolic extract prepared by Soxhlet extraction. Another study by Noumi et al. [50] revealed that the three extracts prepared by cold maceration using solvents such as methanol, ethyl acetate, and acetone for 24 hours are active and present a zone of inhibition that differs depending on the microorganism used and the extract tested. The three extracts methanol, ethyl acetate, and acetone macerates have a zone of inhibition of 13.66, 19.66, and 13.33 mm, respectively, on the strain Staphylococcus aureus ATCC 25923, and they have a zone of inhibition of about 8, 10, and 8 mm on the Pseudomonas aeruginosa strain, while in our study, the acetone macerate showed a zone of inhibition of 11 mm and the diethyl ether macerate showed a zone of 14.5 mm on the Staphylococcus aureus strain CECT976 and a higher zone of inhibition of 18 mm for the acetone macerate on Pseudomonas aeruginosa compared to that obtained with Noumi et al. [ [52,53]. Another study carried out by Pereira et al. [27] on the leaves of J. regia from Portugal intended to test the antimicrobial effect of six walnut trees of different varieties against Gram-positive bacteria (Bacillus cereus, Bacillus subtilis, and Staphylococcus aureus) and Gram-negative bacteria (Pseudomonas aeruginosa, Escherichia coli, and Klebsiella pneumoniae) and whose results showed that Gram-positive bacteria (B. cereus, B. subtilis, and S. aureus) were inhibited by the aqueous extract (Decocted) of the Lara variety at very low concentrations, showing a MIC value of 0.1 mg/mL for B. cereus and S. aureus and a MIC of 10 mg/mL for B. subtilis. Staphylococcus aureus was also inhibited by the Mayette, Parisienne, and Marbot varieties but at a higher extract concentration (1 mg/mL), while Gram-negative bacteria (P. aeruginosa, E. coli, and K. pneumoniae) were less sensitive for the decocted extract of 6 walnut varieties (Lara, Franquette, Mellanaise, Mayette, Parisienne, and Marbot). Indeed, the decocted extract prepared from 6 walnut varieties inhibited bacterial growth by exhibiting a MIC of 100 mg/mL for P. aeruginosa, E. coli, and K. pneumoniae strains, respectively. These results agree with those found by Rather et al. [54] [48].
Our results disagree with the work realized by Senhaji et al. [55] on the antibacterial activity of Anabasis aretioïdes extracts prepared under the same operating conditions and using the same strains, which advanced a total absence of the antibacterial activity of the petroleum ether extract whose polarity is close to that of the diethyl ether used in our study and which gave promising results. Hence, there is a necessity and the interest to have extracts prepared by solvents of different polarities and according to various extraction modalities.
The antibacterial power of all our organic extracts of J. regia bark is explained by the results of the phytochemical study, which revealed the presence of flavonoids, tannins, phenolic compounds, sterols, anthraquinones, quinones, and saponins [23] and whose antimicrobial properties have already been demonstrated [56][57][58][59]. Most of our extracts showed very high flavonoid, tannin, and polyphenol contents, in the first order, the acetone macerated extract whose contents are in the order of 1277:981 ± 2:911 μg QE/mg E, 38:056 ± 1:886 μg CE/mg E, and 327:972 ± 0:06 μg GAE/mg E, respectively, for flavonoids, tannins, and polyphenols [23] which allows us to conclude that flavonoids, tannins, and polyphenols have an antibacterial action, which is in line with the literature, which reported the antimicrobial activity of polyphenols. Among polyphenols, flavan-3-ols, flavonols, and tannins have received the most attention due to their higher antimicrobial activity compared to other polyphenols and the fact that most of them are capable of suppressing several virulence factors such as inhibiting biofilm formation and neutralizing bacterial toxins [60,61].

Principal Component Analysis (PCA).
Principal Component Analysis (PCA) is one of the most widely used descriptive methods for determining correlations between a group of quantitative variables and individuals. The results of the present study revealed that the extracts richer in polyphenols have a better inhibition activity via the alpha-glucosidase test and the inhibition of bacterial growth mainly of the Pseudomonas aeruginosa strain; on the other hand, the extracts rich in tannins presented a better correlation with the 6 microbial strains. The interesting properties of the extracts that are rich in polyphenols and tannins with their antioxidant activities have been reported in our previous work that focused on the analysis of the correlation between flavonoids, tannins, and polyphenols and the five methods used for the evaluation of antioxidant activity (DPPH, RP, ABTS, FRAP, and H 2 O 2 ), from which we found that the extracts richest in polyphenols (acetone macerated and ethanolic macerated) were those that presented the best free radical scavenging activity [23]. The PCA performed by Senhaji et al. on the aqueous and organic extracts of Ajuga iva spp. Pseudoiva from the region of Taza studied by our team under the same experimental conditions also showed a better correlation between the ABTS test of antioxidant activity and polyphenols [62]. These results are in agreement with previous studies that reported that phenolic compounds play an important role in scavenging free radicals and therefore may prevent the onset of diabetes disease [5,43]. Similarly, phenolic compounds have been shown to possess strong antibacterial activity [60]. The better correlation that we obtained of the extracts rich in tannins (diethyl ether macerated and acetone macerated) with the microbial strains Escherichia coli, Proteus mirabilis, Staphylococcus aureus, and Bacillus subtilis can be explained by their antibacterial powers that have been known since the 1990s, where it was demonstrated that these compounds present in green tea (Camellia sinensis) inhibited the growth in vitro of various bacteria, such as Vibrio cholerae, Streptococcus mutans, Campilobacter jejuni, Clostridium perfringes, and Escherichia coli [60].

Conclusion
The present study allowed us to reveal for the first time the mineral composition and hypoglycemic properties via the three tests of inhibition of alpha-amylase, alpha-glucosidase, and beta-galactosidase enzymes of Moroccan Juglans regia bark. In addition, it allowed us to make a comparison of the antibacterial activity of organic extracts of Moroccan J. regia bark prepared by different methods and modalities of extractions with other J. regia harvested in other countries of the world.
At the end of the study of the mineral composition, we can say that J. regia is an important source of mineral elements, with very high contents of Fe (19849. The results of the evaluation of the antidiabetic activity in vitro showed that all the extracts of J. regia bark and in particular the two extracts prepared cold, the aqueous and acetone macerates presented the best activity of inhibition of the enzymes alpha-amylase, alpha-glucosidase, and betagalactosidase. However, the choice of the part of the plant to be tested is a determining factor for pharmacological activity.
For the results of antibacterial activity, the macerated acetone extract at the concentration of 80 mg/mL was found to be the most active by inducing the inhibition zone diameters of 12, 17, 18, 11, 14.5, and 16 mm against Escherichia coli, Proteus mirabilis, Pseudomonas aeruginosa, Staphylococcus aureus, Bacillus subtilis, and Listeria innocua, respectively.
The pharmacological properties of the bark of J. regia are due to the richness of this plant in polyphenols, flavonoids, tannins, anthraquinones, sterols, saponins, and quinones in the bark of J. regia Moroccan [23].
The Principal Component Analysis (PCA) allowed us to find that the best correlations were obtained between the extracts richest in polyphenols and tannins (macerated acetone and macerated diethyl ether) with the tests of the antidiabetic and antibacterial activity.
The results of the present study justified the use of the bark of Juglans regia as an antibacterial and antiseptic agent by the population in the treatment of dental infections.